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Co-phylogeographic structure in a disease-causing parasite and its oyster host

Published online by Cambridge University Press:  21 May 2024

Elizabeth Faye Weatherup*
Affiliation:
Virgina Institute of Marine Science, William & Mary, Gloucester Point, VA, USA Department of Biology and Marine Biology, University of North Carolina Wilmington, Wilmington, North Carolina, USA
Ryan Carnegie
Affiliation:
Virgina Institute of Marine Science, William & Mary, Gloucester Point, VA, USA
Allan E. Strand
Affiliation:
College of Charleston Marine Laboratory and Department of Biology, College of Charleston, Charleston, SC, USA
Erik E. Sotka
Affiliation:
College of Charleston Marine Laboratory and Department of Biology, College of Charleston, Charleston, SC, USA
*
Corresponding author: Elizabeth Faye Weatherup; Email: [email protected]

Abstract

With the increasing affordability of next-generation sequencing technologies, genotype-by-sequencing has become a cost-effective tool for ecologists and conservation biologists to describe a species' evolutionary history. For host–parasite interactions, genotype-by-sequencing can allow the simultaneous examination of host and parasite genomes and can yield insight into co-evolutionary processes. The eastern oyster, Crassostrea virginica, is among the most important aquacultured species in the United States. Natural and farmed oyster populations can be heavily impacted by ‘dermo’ disease caused by an alveolate protist, Perkinsus marinus. Here, we used restricted site-associated DNA sequencing (RADseq) to simultaneously examine spatial population genetic structure of host and parasite. We analysed 393 single-nucleotide polymorphisms (SNPs) for P. marinus and 52,100 SNPs for C. virginica from 36 individual oysters from the Gulf of Mexico (GOM) and mid-Atlantic coastline. All analyses revealed statistically significant genetic differentiation between the GOM and mid-Atlantic coast populations for both C. virginica and P. marinus, and genetic divergence between Chesapeake Bay and the outer coast of Virginia for C. virginica, but not for P. marinus. A co-phylogenetic analysis confirmed significant coupled evolutionary change between host and parasite across large spatial scales. The strong genetic divergence between marine basins raises the possibility that oysters from either basin would not be well adapted to parasite genotypes and phenotypes from the other, which would argue for caution with regard to both oyster and parasite transfers between the Atlantic and GOM regions. More broadly, our results demonstrate the potential of RADseq to describe spatial patterns of genetic divergence consistent with coupled evolution.

Type
Research Article
Creative Commons
Creative Common License - CCCreative Common License - BY
This is an Open Access article, distributed under the terms of the Creative Commons Attribution licence (http://creativecommons.org/licenses/by/4.0/), which permits unrestricted re-use, distribution and reproduction, provided the original article is properly cited.
Copyright
Copyright © The Author(s), 2024. Published by Cambridge University Press

Introduction

Microorganisms with obligate relationships with a host species commonly evolve in response to evolutionary changes in the host, by natural selection (e.g. host resistance or tolerance), or to parallel genetic divergence across biogeographic regions (Van Valen, Reference Van Valen1973; Day, Reference Day1974; Ronquist, Reference Ronquist1997; Page and Charleston, Reference Page and Charleston1998). When host fitness is affected negatively by the presence of parasites, hosts may respond to evolutionary changes in the parasite, thus yielding co-evolutionary dynamics (Thompson, Reference Thompson2005). Co-evolutionary dynamics have significant implications for understanding and managing diseases in ecologically and economically important species (Coen and Bishop, Reference Coen and Bishop2015). Parasite tracking of host evolution, co-evolution or both yield significant patterns of coupled evolution between host and parasite genomes over space and time that can be quantified using emerging genotyping technologies (Vermeer et al., Reference Vermeer, Dicke and De Jong2011).

Most previous efforts to study coupled evolution of host–parasite interactions using genetics utilized microsatellites or Sanger sequencing of a 1 or a few loci, which is relatively time-consuming and expensive on a per-locus basis (Ebert and Fields, Reference Ebert and Fields2020; Märkle et al., Reference Märkle, John, Cornille, Fields and Tellier2021). Recent advances in simultaneously amplifying single-nucleotide polymorphisms (or SNPs) using high-throughput sequencing technologies have allowed scientists the opportunity to use genotype-by-sequencing for both host and parasite genomes simultaneously. For example, Choi et al. (Reference Choi, Aliota, Mayhew, Erickson and Christensen2014) used dual RNA sequencing to simultaneously look at Brugia malayi larvae and its mosquito host. Ansari et al. (Reference Ansari, Pedergnana, Ip, Magri, Von Delft, Bonsall, Chaturvedi, Bartha, Smith, Nicholson, McVean, Trebes, Piazza, Fellay, Cooke, Foster, Hudson, McLauchlan, Simmonds, Bowden, Klenerman, Barnes and Spencer2017) used a genome-wide association study (GWAS) of individuals infected with hepatitis C virus to show how SNPs in both the virus and host impacted the infection progression. Another study by Lees et al. (Reference Lees, Ferwerda, Kremer, Wheeler, Serón, Croucher, Gladstone, Bootsma, Rots, Wijmega-Monsuur, Sanders, Trzciński, Wyllie, Zwinderman, van den Berg, van Rheenen, Veldink, Harboe, Lundbo, de Groot, van Schoor, van der Velde, Ängquist, Sørensen, Nohr, Mentzer, Mills, Knight, du Plessis, Nzenze, Weiser, Parkhill, Madhi, Benfield, von Gottberg, van der Ende, Brouwer, Barrett, Bentley and van de Beek2019) also used GWAS to look at genomes of human hosts and Streptococcus pneumoniae, finding that host SNP variation is significant in differences in susceptibility to this bacterium. Most recently, Dexter et al. (Reference Dexter, Fields and Ebert2023) conducted a co-genome study of the planktonic crustacean, Daphnia magna, and its parasite Pasteuria ramosa, an endoparasitic bacterium (Dexter et al., Reference Dexter, Fields and Ebert2023). They found a signal of interspecies linkage disequilibrium across multiple sets of loci demonstrating the coevolution of this host and parasite system (Dexter et al., Reference Dexter, Fields and Ebert2023). Additionally, there have been several studies that have used restricted site-associated DNA sequencing (RADseq) to characterize host and parasite systems. Bracewell et al. (Reference Bracewell, Vanderpool, Good and Six2018) used RADseq to find evidence of co-evolution and cascading speciation among 4 close interacting species, the western pine beetle, Dendroctonus brevicomis, the beetle's mutualistic fungi, Ceratocystiopsis brevicomi and Entomocorticium sp., and the beetle's host tree, Pinus ponderosa (Bracewell et al., Reference Bracewell, Vanderpool, Good and Six2018). Another study by Satler et al. (Reference Satler, Herre, Jandér, Eaton, Machado, Heath and Nason2019) was able to determine the frequent phenomena of host switching in Panamanian strangler figs and their pollinating fig wasps (Satler et al., Reference Satler, Herre, Jandér, Eaton, Machado, Heath and Nason2019). A similar occurrence was found in a study by Sweet et al. (Reference Sweet, Wilson, Sonsthagen and Johnson2020). Sweet et al. used whole-genome sequencing and double-digested RADseq to obtain SNPs to examine co-evolutionary patterns and host-switching accessibility between 2 species of ptarmigan birds and their associated feather lice parasites, Lagopoecus and Goniodes. They found evidence of frequent host switching of lice among different bird populations in Alaska, as well as co-evolutionary patterns between the lice and birds (Sweet et al., Reference Sweet, Wilson, Sonsthagen and Johnson2020).

The alveolate parasite Perkinsus marinus (Ph. Perkinsozoa) infects the eastern oyster Crassostrea virginica (Ph. Mollusca) along much of the oyster's geographic range from the Gulf of St. Lawrence, Canada to the Gulf of Mexico (GOM; Sparks, Reference Sparks1966). In addition to its ecological importance (Zimmerman et al., Reference Zimmerman, Minello, Baumer and Castiglione1989; Smaal and Prins, Reference Smaal, Prins and Dame1993), C. virginica has been the focus of historically as well as contemporarily significant fisheries and aquaculture industries. Perkinsus marinus causes ‘dermo’ disease, which can lead to widespread mortality in oyster populations (Carnegie et al., Reference Carnegie, Ford, Crockett, Kingsley-Smith, Bienlien, Safi, Whitefleet-Smith and Burreson2021). Because of its significance, P. marinus has been a primary focus of regulation of aquaculture products among states of the US East Coast and the GOM, but the effectiveness of these regulations would benefit from deeper understanding of the ecological and evolutionary relationships between this host and parasite. To our knowledge, however, no previous genetic studies of P. marinus have genotyped SNPs nor simultaneously examined the oyster and parasite population genetics within the same individuals.

Unlike most other protozoans infecting molluscs, P. marinus can be cultured in vitro, which has made more analyses possible of the phenotypic and genetic structure of this parasite across its distribution than for other oyster parasites. In seminal early work, Bushek and Allen (Reference Bushek and Allen1996) found that Atlantic isolates (VA and NJ) were more virulent than isolates from the GOM coast (TX and LA) in oysters collected from all 4 populations. Reece et al. (Reference Reece, Bushek and Graves1997, Reference Reece, Bushek, Hudson and Graves2001) genotyped restriction fragment length polymorphisms of in vitro cultures of P. marinus, noted the presence of diploid or multiple infections of P. marinus in single oysters and revealed 3 genetically distinct subdivisions among estuaries of the United States: the northeast Atlantic, southeast Atlantic and GOM (Reece et al., Reference Reece, Bushek and Graves1997, Reference Reece, Bushek, Hudson and Graves2001). Thompson et al. (Reference Thompson, Rosenthal and Hare2011, Reference Thompson, Rosenthal and Hare2014) genotyped microsatellite markers and demonstrated the presence of dimorphic loci suggesting an ancient hybridization event that persists and a fairly complex, non-equilibria pattern of spatial population structure along the Atlantic and GOM coastlines (Thompson et al., Reference Thompson, Rosenthal and Hare2011, Reference Thompson, Rosenthal and Hare2014).

Phylogeographic divergence among C. virginica populations is also well described. Multiple studies using a variety of mitochondrial and nuclear loci (Reeb and Avise, Reference Reeb and Avise1990; Hare and Avise, Reference Hare and Avise1996; Varney et al., Reference Varney, Galindo-Sánchez, Cruz and Gaffney2009; Thongda et al., Reference Thongda, Zhao, Zhang, Jescovitch, Liu, Guo, Schrandt, Powers and Peatman2018) have indicated divergence among and within the United States coastline of the GOM and Atlantic. These patterns reflect likely relatively short larval period (<2 weeks), entrainment of larvae within estuaries and possibly local purifying selection (Murray and Hare, Reference Murray and Hare2006; Burford et al., Reference Burford, Scarpa, Cook and Hare2014).

Here, we used RADseq to examine SNPs of P. marinus and C. virginica within P. marinus-infected oysters. Our sampling was focused on infected adults collected at 2 GOM locations (Dauphin Island, AL, and Caminada Bay, LA) and Atlantic coast locations in Virginia (Great Wicomico River, Mockhorn Bay, York River, Burtons Bay, James River and Rappahannock River). We expected a parallel phylogeographic divergence in oyster and parasite genomes from the Gulf and Atlantic coasts yielding a significant co-phylogenetic signal partitioned across the geography of this host–parasite system.

Methods

Collection

We genotyped 95% ethanol-preserved oyster samples from Maryland (1 location), Virginia (14 locations), Alabama (1 location) and Louisiana (2 locations), as well as an in vitro culture of P. marinus originally collected in Galveston Bay, Texas, and 1 paraffin-embedded sample initially preserved in Davidson's fixative (Shaw and Battle, Reference Shaw and Battle1957) (Table 1). The Virginia samples were collected during routine surveillance for oyster diseases conducted by the Carnegie lab at the Virginia Institute of Marine Science (VIMS). Samples from other states represented aquaculture industry samples submitted for disease analysis in the context of interstate shellfish commerce. For each oyster sampled, animals were cleaned, measured and shucked to expose soft tissues. Gill and mantle were extracted from each oyster and preserved in 95% ethanol for genetic analysis.

Table 1. Oyster populations that were positive for P. marinus and extracted and sequenced [AL (n = 3), LA (n = 9), VA Bay (n = 18), VA Eastern (n = 6)].

Identification of oysters positive for Perkinsus marinus

DNA was extracted using a QIAGEN QIAamp DNA Mini Kit. Genomic DNA concentration was measured with a Nanodrop spectrophotometer to ensure the concentration was ≥100 ng μL−1. If the concentration was >300 ng  μL−1, then the DNA was diluted in an equal volume of Milli-Q® water before polymerase chain reaction (PCR). A concentration of about 100 ng  μL−1 was considered optimum for amplification of P. marinus-specific primers in each oyster sample. Samples were run on a PCR using PmarITS-70 forward primer (5′-CTT TTG YTW GAG WGT TGC GAG ATG-3′) and PmarITS-600 reverse primer (5′-CGA GTT TGC GAG TAC CTC KAG AG-3′), which target P. marinus. Denaturing was done at 94 °C for 30 s, annealing at 57 °C for 30 s and extension at 72 °C for 1.5 min. These steps were repeated 40 times. After PCR, to identify oysters that were positive for P. marinus, the PCR products were run on a 2% agarose gel at 100 volts for 30 min and stained with GelRed Nucleic Acid stain in a water bath for 25 min. This included a 1KB bp ladder at the first lane of the gel so that the desired 1000 base pair size could be visualized. Positive samples were identified and used for further analysis. The goal was to obtain 30 positive samples for each site, which was possible in some cases, but not all.

All positive samples in microcentrifuge tubes were randomly mixed before transport in case there was an error in future sequencing steps that could cause a loss in representation of an entire population. Once the microcentrifuge tubes containing the extracted DNA were thoroughly mixed, 20 μL of each of the 64 samples were used in subsequent library construction.

Library preparation

We prepared genomic libraries using the genotype-by-sequencing approach outlined in Parchman et al. (Reference Parchman, Gompert, Mudge, Schilkey, Benkman and Buerkle2012), applied to samples identified as P. marinus-positive. The DNA of each individual oyster was digested separately with 2 restriction enzymes, EcoRI and MseI. The digested DNA fragments were then ligated to Illumina adaptors at the MseI end and with Illumina adaptors coupled with an 8–10 bp unique barcode to the EcoRI end to allow identification of the individual in silico. The restriction-ligation products were then PCR-amplified in 2 separate reactions using standard Illumina primers. The final PCR products were pooled and shipped for sequencing.

Fifty-nine P. marinus-positive samples were sequenced in 2020 at the Tufts University Genomic Services (200–400 bp fraction; single-end sequencing on an Illumina HiSeq 2500 using SE125), 42 samples were sequenced in 2022 at the University of Texas Genomic Sequencing and Analysis Facility (300–450 bp fraction; single-end sequencing on an Illumina NovaSeq SP using SR100) and 37 of each of those samples were sequenced in both runs.

Data filtering

Reads were aligned to the P. marinus genome (GCA_000006405.1) using bwa mem (Li and Durbin, Reference Li and Durbin2010) and samtools/bcftools 1.9 (Danecek et al., Reference Danecek, Bonfield, Liddle, Marshall, Ohan, Pollard, Whitwham, Keane, McCarthy, Davies and Li2021) using default settings. We also aligned these samples to the C. virginica genome (GCF_002022765.2). The median number of reads aligned to the P. marinus genome (0.13 M; a range of 0.10–1.01 M) was 0.37% of the median number aligned to the C. virginica genome (34 M; a range of 3.52–66.89 M). This yielded a ratio of 265 C. virginica to P. marinus reads per sample. Of the total number of reads per sample, a median of 0.80 and 91.30% of reads were P. marinus and C. virginica, respectively.

After alignment of 64 samples to the P. marinus genome, we kept 35 samples that had between 100 K and 1 M P. marinus reads. Another sample identified as 6837–16, from VA had 1.1 M reads, from which we randomly downsampled 500 K reads using samtools view. A final sample of 1993 TX live culture (TX-2-69, purchased from the American Type Culture Collection, ATCC) had 25 million reads that aligned with P. marinus; however, genotype calls showed a predominance of no calls (NAs) and consequently, it was removed. One likely reason for NAs at this step is that this culture contains multiple strains that interfere with genotype calling algorithms. For the remainder of the samples, we did not detect the presence of multiple strains nor patterns of dimorphic loci (Thompson et al., Reference Thompson, Rosenthal and Hare2014). Thus, we were left with 36 samples (Table 1).

For P. marinus, we used bcftools to find all SNPs [set minor allele frequency (MAF) threshold at 0] and then a custom script to find SNPs that had at least 1 read across 50% of individuals. This yielded 772 SNPs. An analysis of allele frequencies using angsd (-doMAF 1) indicated that 393 SNPs were polymorphic between or within samples. Thus, all subsequent analyses are based on samtools-generated phred-scale genotype likelihoods of 393 polymorphic SNPs at 36 individuals. For C. virginica, we created genotypes from the same 36 individuals, and included SNPs with MAF > 1% and at least 1 read per sample, yielding samtools-generated genotypes at 52 100 SNPs.

Principal component analysis

Principal component analysis (PCA) plots were generated for both organisms between collections. We used PCangsd (Meisner and Albrechtsen, Reference Meisner and Albrechtsen2018) on P. marinus genotype likelihoods and prcomp on C. virginica genotype calls within R (R Core Team, 2021). PCA is an exploratory analysis for large datasets providing more comprehensible information by grouping the data based on the individual samples' genotypic similarities.

Analysis of molecular variance

To assess how much genetic variation is partitioned among and within groups of samples, we performed hierarchical analysis of molecular variance (AMOVA; Excoffier et al., Reference Excoffier, Smouse and Quattro1992) using Pegas (Paradis, Reference Paradis2010). P values were generated using 1000 bootstrap replicates. For P. marinus, we converted the phred-scale genotype likelihoods per SNP-sample combination into probabilities that summed to 1 and then converted these to a single value ranging from 0 to 2, where 0, 1 and 2 represent the highest probability of a homozygote, heterozygote and alternative homozygote, respectively. This matrix served as an input to Pegas. For C. virginica, the input was genotype calls from samtools pulled using R:vcfR (Knaus and Grünwald, Reference Knaus and Grünwald2017) from a vcf file. Given the patterns found in PCA, we analysed 4 groups of samples: Alabama (n = 3), Louisiana (n = 9), Virginia Chesapeake Bay (n = 18) and Virginia Eastern Shore seaside (n = 6; see Table 1). We estimated expected heterozygosity in P. marinus using genotype likelihoods as implemented in angsd, and of genotype calls in C. virginica using strataG (Archer et al., 2016).

Admixture analysis

We implemented maximum-likelihood admixture methods to infer ancestry of individuals. We used NGSadmix (Meisner and Albrechtsen, Reference Meisner and Albrechtsen2018) to analyse genotype likelihoods of P. marinus and LEA: SNMF (Frichot and François, Reference Frichot and François2015) to analyse genotype calls of C. virginica. Analyses were run across an a priori range of genetic clusters (k = 2–10) and replicated 10 times. Given the low number of samples, we only visualized up to k = 6 for both datasets. An analysis of logL changes (following Evanno et al., Reference Evanno, Regnaut and Goudet2005) indicates that the best-fit k to the P. marinus dataset was k = 5. The strongest cross-validation in the SNMF C. virginica analysis was k = 6.

Co-phylogenetic analysis

We visualized the co-phylogenetic structure between host and parasite using maximum-likelihood trees. We first generated fasta-formatted files of concatenated SNPs coded as IUPAC nucleotides using seqinr (Charif and Lobry, Reference Charif, Lobry, Bastolla, Porto, Roman and Vendruscolo2007). For P. marinus, we used PhyML implemented in SeaView (Gouy et al., Reference Gouy, Guindon and Gascuel2010) with default parameters (GTR + 4 rate classes as a model of evolution; 100 bootstrap replicates). For C. virginica, we used IQTree (Trifinopoulos et al., Reference Trifinopoulos, Nguyen, von Haeseler and Minh2016), which had 12766 parsimony-informative and 10028 singleton SNPs. The best-fit model of evolution was TVM + F + I + G4, allele frequencies were computed from the alignment and we used the ultrafast method to create 1000 bootstrap replicates. To statistically assess cophylogenetic signal among host and parasite, we used these trees as input to the Procrustean Approach to Co-phylogeny, or R::paco (Hutchinson et al., Reference Hutchinson, Cagua, Balbuena, Stouffer and Poisot2017). This approach assumes dependence of the parasite phylogeny on host, and assesses the probability that the observed network has more phylogenetic congruence than 1000 random instances of the interaction network (Fig. 1).

Figure 1. Map of geographic location of each site collection for the region of Virginia [circle, Chesapeake Bay; squares, Eastern Shore; red, Fleet Point (n = 2); yellow, VIMS Beach (n = 11); orange, Wreck Shoal (n = 1); black, Broad Creek (n = 1); purple, Wachapreague (n = 1); blue, Oyster (n = 6)] and 2 regions in the Gulf of Mexico [red = Louisiana (n = 5) and black = Alabama (n = 3)].

Results

Strong genetic divergence between the GOM collections (LA and AL) and Virginia were revealed within the nuclear genomes of both P. marinus and C. virginica in all analyses. PCA (Fig. 2), admixture analyses (Fig. 3) and an AMOVA (Table 2) revealed strong divergence in P. marinus and C. virginica genotypes.

Figure 2. Principal components analyses of (A) Perkinsus marinus (393 loci, n = 36) from PCangsd and (B) Crassostrea virginica (52100 SNPs, n = 35) from prcomp.

Figure 3. Admixture analysis of (A) Perkinsus marinus (393 loci, n = 36) using genotype likelihoods in NGSadmix and (B) Crassostrea virginica (52100 SNPs, n = 35) using genotypes in SNMF.

Table 2. Analysis of molecular variance (AMOVA) on Perkinsus marinus and Crassostrea virginica samples

Overall PhiST (i.e. across 4 populations) was 0.125 (P = 0.005) and 0.165 (P < 0.001) for P. marinus and C. virginica, respectively. Pairwise-PhiST values are shown below and above diagonals, respectively.

In contrast, there was discordance between host and parasite in geographic divergence at smaller spatial scales within Virginia. Crassostrea virginica genotypes between Chesapeake Bay and seaside Eastern Shore groups were divergent in PCA (Fig. 2B), admixture (Fig. 3B) and AMOVA (Table 2). However, P. marinus genotypes were not clearly divergent in any of these analyses (Figs 2A, 3A and 4; Table 2). Regions also did not differ in expected heterozygosity for either P. marinus or C. virginica (Table 3).

Figure 4. A maximum-likelihood co-phylogeny of the parasite Perkinsus marinus (392 bp) and host Crassostrea virginica (52052 bp). All nodes have 100% consensus support for C. virginica while all nodes have <50% support for P. marinus (1000 bootstrap replicates for both). Black and red dashed lines indicate GOM and VA genotypes within Crassostrea, respectively, and linked to Perkinsus genotypes.

Table 3. Expected heterozygosity (mean ± standard error across individuals) for Crassostrea virginica and Perkinsus marinus

A co-phylogeny plot (Fig. 4) provides a view of both the phylogeographic structure and patterns of mixing between host and parasite genotypes. Overall, paco (Hutchinson et al., Reference Hutchinson, Cagua, Balbuena, Stouffer and Poisot2017) indicated a significant co-phylogenetic signal between the groups (m2xy = 0.180, P < 0.001, n = 1000). Thus, across all samples, the parasite phylogeny significantly tracked the oyster phylogeny, indicating they have undergone coupled evolutionary change, at least at the larger GOM vs Atlantic spatial scale. There were 2 oyster samples collected in GOM (coded LA6946-C and AL7040-6) that had P. marinus genotypes that were embedded within the Virginia clade (Fig. 4). This may have reflected ancestral polymorphisms from a single ancestor that have not been sorted, poor phylogenetic support in the ML tree of the P. marinus or more recent movement of P. marinus from the Atlantic to the GOM.

Discussion

In our analyses, clear genotypic differentiation was evident between our Atlantic samples and those from the GOM, in both P. marinus and C. virginica (Figs 2 and 3; Table 2). Furthermore, we identified genotypic differentiation within C. virginica populations between the Chesapeake Bay and the seaside Eastern Shore in Virginia (Figs 2 and 3; Table 2). These findings support previous research on P. marinus (Reece et al., Reference Reece, Bushek and Graves1997, Reference Reece, Bushek, Hudson and Graves2001; Thompson et al., Reference Thompson, Rosenthal and Hare2014) that documented the genetic differentiation of P. marinus between the GOM and Mid-Atlantic regions. It is worth noting that expanding our sampling of individuals and loci could potentially unveil significant genetic structure of P. marinus populations within regions. Our results also align with the conclusions of Varney et al. (Reference Varney, Galindo-Sánchez, Cruz and Gaffney2009) and Thongda et al. (Reference Thongda, Zhao, Zhang, Jescovitch, Liu, Guo, Schrandt, Powers and Peatman2018) for C. virginica, of genetic differentiation between and within regions. This strong genetic structure within regions likely reflects barriers to larval dispersal, local selection or both (Stauber, Reference Stauber1950; Narváez et al., Reference Narváez, Klinck, Powell, Hofmann, Wilkin and Haidvogel2012).

Our maximum-likelihood analysis (Fig. 4) revealed a strong signal of co-phylogeny between the parasite P. marinus and its oyster host. A close interaction between these 2, documented for nearly three-quarters of a century but potentially of far older origins, has resulted in an ongoing arms race, as these organisms are continually adapting to outcompete one another. This phenomenon is observed in numerous other species (Dismukes et al., Reference Dismukes, Braga, Hembry, Heath and Landis2022), and this methodology has the potential to uncover a multitude of evolutionary histories between hosts and parasites across diverse species.

This approach enabled us to detect genetic structure between the GOM and Atlantic P. marinus populations, which underscores its potential effectiveness to resolve the regional genetic diversity more finely in this pathogen. The implications for management of P. marinus in the context of regional shellfish aquaculture commerce are already important, even if this initial analysis was too limited to provide clear perspective on intra-regional diversity. Resource managers in the states affected by P. marinus parasitism of oysters are keenly interested in the question of genetic structure, because of the possibility of inadvertently creating new encounters, by pathogen introduction from distant waters through aquaculture transfers, between local oysters and P. marinus ‘strains’, or phenotypes, to which local oyster populations are not well adapted. The concern is that this would potentially result in a P. marinus epizootic of increased severity and economic destruction. Even if P. marinus is widely distributed and widely similar in prevalence across locations, which would argue that any aquaculture transfer of oysters with a low prevalence of P. marinus infections should be inconsequential against the natural backdrop of highly prevalent P. marinus, there is an increasing reluctance to risk introductions of P. marinus along with shellfish transfers because of genetic concerns. Better resolution of P. marinus genetic (and ideally, phenotypic) diversity could allow determination of ‘zones’ of common genotypic and phenotypic profiles within which control of P. marinus in transfers might be relaxed, to the benefit of reasonable aquaculture commerce and aquaculture biosecurity generally (Bushek and Allen, Reference Bushek and Allen1996; Reece et al., Reference Reece, Bushek and Graves1997, Reference Reece, Bushek, Hudson and Graves2001; Carnegie et al., Reference Carnegie, Arzul and Bushek2016). Based on our analyses, a case could already be made that divergence between Atlantic and GOM P. marinus populations would suggest that they should be precautionarily managed as distinct ‘zones’, between which transfers of allopatric parasite as well as oyster genotypes and phenotypes should be avoided.

This study also resulted in analysis among 393 SNPs for the parasite, despite the samples being dominated by host DNA, as it was taken from a gill and mantle sample from each oyster. The analyses were able to be examined at 52 100 SNPs for the host genome, C. virginica, demonstrating that with a high alignment of reads to the genome, this method can yield deep sequencing analysis, which is necessary to providing fine resolution of population genetics of species to aid in disease and risk management (Bernatchez et al., Reference Bernatchez, Xuereb, Laporte, Benestan, Steeves, Laflamme, Bernatchez and Mallet2019).

Future steps

The process of uncovering multiple loci simultaneously for both host and parasite species through RADseq and Illumina sequencing holds immense promise for future population genetic studies. However, it is important to acknowledge the limitations of our analysis, primarily stemming from the relatively small sample size and limited sample locations. To enhance the utility of this tool for co-phylogeny studies, several steps can be taken, especially regarding the parasite analysis.

First, expanding the sample size from each location to include a minimum of 30 or more P. marinus-positive oysters would strengthen the robustness of our analyses. This larger dataset would provide a more comprehensive understanding of the genetic structure of the parasite within and across regions, potentially allowing us to identify unique genotypes with important implications for management strategies. Another improvement involves finding a method to enrich parasite DNA, as it is significantly overshadowed by host DNA. This could be achieved by incorporating a pre-amplification step utilizing beads with attached oligonucleotides designed to specifically target the desired parasite loci, a technique supported by prior research (Shapero et al., Reference Shapero, Leuther, Nguyen, Scott and Jones2001; Rödiger et al., Reference Rödiger, Liebsch, Schmidt, Lehmann, Resch-Genger, Schedler and Schierack2014). Through the application of such amplification methods and an increased sample size, we could gain deeper insights into the genetic structure of the parasite.

Conclusion

This study highlights genotypic divergence among regions and within regions of P. marinus and its host, C. virginica using RADseq. Unlike other studies (Bracewell et al., Reference Bracewell, Vanderpool, Good and Six2018; Satler et al., Reference Satler, Herre, Jandér, Eaton, Machado, Heath and Nason2019; Sweet et al., Reference Sweet, Wilson, Sonsthagen and Johnson2020) that used RADseq, this study amplified genomes of both host and parasites from a naturally infected host, rather than a lab infection or separate sequencing. This allowed us to get an accurate and current view on the evolutionary interactions in this host and parasite system. Moreover, RADseq offers a straightforward means of assessing coupled evolutionary change within host and parasite species simultaneously.

This study could be improved with an increased sampling size of wild oysters, more sampling sites and a method to increase parasite loci. However, despite the low sampling size, this methodology provided us insight into this host parasite interaction effectively.

Data availability statement

Relevant code and datasets are found at https://github.com/esotka/WeatherupPerkinsus. FASTQ files have been uploaded to GenBank (BioSample accession SAMN39856659–95).

Author contributions

All authors conceived and designed the study and edited the final manuscript. R. C. and E. F. W. collected samples, and E. F. W. extracted samples. E. F. W. and E. E. S. prepared the samples for sequencing, performed all analyses, generated figures and tables and wrote the manuscript.

Financial support

This research was funded by the National Science Foundation (OCE-1924599) and the VIMS Foundation A. Marshall Acuff, Sr., Memorial Endowment for Oyster Disease Research.

Competing interests

None.

Ethical standards

Not applicable.

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Figure 0

Table 1. Oyster populations that were positive for P. marinus and extracted and sequenced [AL (n = 3), LA (n = 9), VA Bay (n = 18), VA Eastern (n = 6)].

Figure 1

Figure 1. Map of geographic location of each site collection for the region of Virginia [circle, Chesapeake Bay; squares, Eastern Shore; red, Fleet Point (n = 2); yellow, VIMS Beach (n = 11); orange, Wreck Shoal (n = 1); black, Broad Creek (n = 1); purple, Wachapreague (n = 1); blue, Oyster (n = 6)] and 2 regions in the Gulf of Mexico [red = Louisiana (n = 5) and black = Alabama (n = 3)].

Figure 2

Figure 2. Principal components analyses of (A) Perkinsus marinus (393 loci, n = 36) from PCangsd and (B) Crassostrea virginica (52100 SNPs, n = 35) from prcomp.

Figure 3

Figure 3. Admixture analysis of (A) Perkinsus marinus (393 loci, n = 36) using genotype likelihoods in NGSadmix and (B) Crassostrea virginica (52100 SNPs, n = 35) using genotypes in SNMF.

Figure 4

Table 2. Analysis of molecular variance (AMOVA) on Perkinsus marinus and Crassostrea virginica samples

Figure 5

Figure 4. A maximum-likelihood co-phylogeny of the parasite Perkinsus marinus (392 bp) and host Crassostrea virginica (52052 bp). All nodes have 100% consensus support for C. virginica while all nodes have <50% support for P. marinus (1000 bootstrap replicates for both). Black and red dashed lines indicate GOM and VA genotypes within Crassostrea, respectively, and linked to Perkinsus genotypes.

Figure 6

Table 3. Expected heterozygosity (mean ± standard error across individuals) for Crassostrea virginica and Perkinsus marinus